海绵特异性微生物的分子钟初测及其意义

海绵动物是最原始的后生动物,营底栖、滤食性生活,它们体内共生有丰富的微生物菌落,包括仅在海绵动物体内存在的特异性微生物。为了探讨海绵特异微生物是否与宿主存在协同演化关系,我们基于16SrRNA基因序列利用宽松分子钟方法估测了各个门类中海绵特异微生物的分歧时间,并与海绵动物的化石记录及分子谱系年代学结果相比较。结果表明:多数微生物门类中海绵特异微生物的分支分化发生在新元古代(800—1000Ma),与海绵动物的分子化石记录和当前分子钟估算结果之间存在一定程度的一致性,说明微生物与宿主海绵动物之间存在一定的协同演化关系。少数门类中海绵特异微生物分化时间过早于(如蓝细菌,2200Ma)或者过晚于(如古细菌,148Ma;Alphaproteobacteria,480Ma)新元古代,这可能是由于系统采样等因素所致,有待于进一步的分析与研究。     

棘尾虫类神经肽的免疫细胞化学研究

用光镜、电镜免疫组织化学方法,在原生动物棘尾虫(Stylonychia mytilus)体内发现多种哺乳动物神经肽、肽激素和酪氨酸羟化酶免疫阳性物质:类P 物质(SP-Like),类神经肽Y(NPY-Like),类胆囊收缩素(CCK-8-Like),类生长抑素(SOM-Ljke),类β-内啡肽(β-end-orphin-Ljke),类促肾上腺皮质激素(ACTH-Like)和类酪氨酸羟化酶(TH-Like)。免疫细胞化学实验显示了这些肽类免疫阳性物质的分布。     

动物的毛与人发角蛋白组分的比较研究

本文用SDS-聚丙烯酰胺凝胶电泳(SDS-PAGE)对10科18种50份动物毛与人发进行了角蛋白组分分析。结果证实,动物的毛与人发角蛋白组分的主要差异在<18.500低分子量区域;不同种属的动物毛角蛋白组分也存在明显差异;大熊猫毛的角蛋白组分与小熊猫和黑熊的相比有显著不同。不同种属动物毛角蛋白组分的差异对动物分类学研究能提供有参考价值的实验依据。     

两种中国南海海绵的化学成分和生物活性研究

本文对采自中国南海的两种海绵(Petrosia sp.和Haliclona sp.)进行了系统的化学成分研究,综合利用各种层析技术(硅胶柱层析、凝胶柱层析)从中分离纯化出14个化合物,并利用波谱技术(IR、UV、NMR)对其结构进行了鉴定。从石海绵(Petrosia sp.)中分离的化合物为:3-isocyanotheonellin(1)、theonellin isothiocyanate(2)、theonellin amine(3)、theonellin formamide(4)和邻苯二甲酸二异丁酯(5);从蜂海绵(Haliclona sp.)中分离的化合物为:renierol(6)、isoquinolinequinones mimosamycin(7)、胆甾醇(8)、麦角甾醇(9)、(24R)-ergosta-7,22-diene-3β,5β,6β-triol(10)、5α,8α-epidioxycholest-6-en-3β-ol(11)、胸苷(12)、胞苷(13)、鲨烯(14)及邻苯二甲酸二异丁酯(5)。在对化合物进行广泛的生物活性筛选时发现:化合物6能有效抑制黄嘌呤氧化酶。化合物1～7,9～10,14是首次从该两种海绵中分离得到。     

快速膨胀片层多孔壳聚糖止血海绵的制备及生物相容性研究

目的:探索快速膨胀片层多孔壳聚糖止血海绵的制备工艺,评价止血海绵的理化性能及生物相容性,并探讨原料脱乙酰度对止血海绵性能的影响。方法:考察止血海绵的理化性质,包括扫描电子显微镜(SEM)观察表观形貌,检测力学性能、吸水率、快速吸水膨胀时间和膨胀率,研究其体内外的生物相容性,包括体外细胞毒性实验、动物皮内刺激实验和皮下植入实验。结果:确定了止血海绵的制备工艺,采用该工艺制备的止血海绵均具有片层多孔结构,且具有较高的力学强度和快速膨胀的特点。证实高脱乙酰度原料(DD=95.14%)制备的止血海绵力学性能、吸水率、膨胀率均优于低脱乙酰度原料(DD=69.70%)制备的止血海绵。脱乙酰度69.70%和脱乙酰度95.14%的壳聚糖止血海绵,拉伸强度分别为10.1 N和15.4 N,吸水率分别为1904%和2131%,吸水膨胀时间分别为13.4 s和14.0 s,膨胀率分别为8.4倍和10.8倍。体外细胞毒性实验表明脱乙酰度为95.14%的壳聚糖止血海绵更有利于细胞的增殖,皮内刺激和皮下植入实验结果表明脱乙酰度为95.14%的壳聚糖海止血海绵表现出更小的组织炎性反应。结论:脱乙酰度为95.14%的壳聚糖止血海绵具有优良的力学性能、优异的吸水膨胀能力以及良好的生物相容性,在临床止血特别是腔隙止血方面具有广阔的应用前景。     

生后雌性小鼠下丘脑室旁核内ER-β表达的免疫组化研究

研究发现小鼠下丘脑室旁核(PVN)内雌激素β受体(ER-β)的表达与在大鼠等一些实验动物脑PVN的表达有差异,提示其在小鼠PVN内的表达可能有特定的生理意义。为了深入探讨ER-β在小鼠PVN内的功能,本文采用硫酸镍铵增强显色的免疫组化SP法研究了ER-β在生后雌性小鼠PVN内的表达。结果发现ER-β免疫阳性物质主要见于PVN的大细胞部,在小细胞部和背侧帽部免疫阳性细胞数目较少。免疫阳性物质主要位于细胞核内,未发现明显的胞浆或突起阳性,但在发育的某些时期可见免疫阳性细胞核局部呈现阴性反应。最高表达见于生后早期(第1-9天),随后表达降低,生后一个月即达到成年水平。PVN内ER-β的表达模式表现为生后早期表达高、随后降低,提示在该部位ER-β可能主要参与了对生后早期PVN的神经内分泌活动以及神经结构的发育与完善的调控,并可能与生后早期动物的应激、体重增加和脂肪代谢等有关。     

类鼻疽伯克霍尔德菌bopA基因敲除株的构建及生物学特征

【【背景】类鼻疽杆菌是一种能够引起人类疾病甚至死亡的胞内寄生菌,Ⅲ型分泌系统在该菌入侵上皮细胞、逃避宿主免疫以及毒力因子的分泌过程中发挥重要作用,其中bopA基因为TTSS-3基因编码的重要效应蛋白,在类鼻疽杆菌的免疫逃逸中发挥重要作用。【目的】构建类鼻疽杆菌bopA基因敲除菌株,并对其生物学特征进行初步研究。【方法】构建pK18mobSacB-ΔbopA自杀质粒,通过大肠杆菌S17-1λpair以接合的方式转入类鼻疽杆菌,利用同源重组敲除了bopA基因,并用蔗糖平板筛选出菌株,最后在细胞和动物水平检测敲除菌株的表型变化。【结果】构建了bopA敲除的类鼻疽菌株,并通过细胞和动物实验证实敲除bopA基因后,细菌的细胞侵袭和胞内存活以及体内定殖能力都显著降低。【结论】利用同源重组成功构建类鼻疽bopA基因敲除株,为深入研究该基因的作用靶点奠定了实验基础。     

稳定表达β-synuclein的SH-SY5Y细胞株的构建

目的构建稳定表达β-synuclein的SH-SY5Y细胞株。方法利用脂质体转染技术将质粒pcD-NA3.1-β-synuclein转染SH-SY5Y细胞,通过Zeocin进行抗性筛选。采用原位免疫荧光、免疫组织化学染色及Western blot杂交检测β-synuclein在SH-SY5Y细胞中的表达情况;通过MTT比色法检测β-synuclein稳定表达对SH-SY5Y细胞增殖的影响。结果原位免疫荧光、免疫组织化学染色及Western blot检测结果显示β-synuclein在SH-SY5Y细胞中的表达水平较对照组明显升高;稳定表达β-synuclein的细胞增殖程度较对照组明显增高(P<0.05)。结论β-synuclein在SH-SY5Y细胞中稳定表达,为后续的研究提供有用的细胞模型。为进一步研究β-sy-nuclein对帕金森病发病神经保护作用的研究奠定了良好的基础。     

陕西镇巴早寒武世海绵骨针化石

作者对采自陕西省镇巴县下寒武统西蒿坪段和水井沱组下部碳酸盐岩地层的海绵骨针化石进行了研究。三叶虫及小壳化石的生物地层学资料表明西蒿坪段和水井沱组下段属于筇竹寺阶。化石经室内醋酸浸泡处理后获得,骨针化石保存较好、类型多样,其中属于六射海绵纲的骨针3类,普通海绵纲的骨针6类,分类未定的骨针1类(Nabaviellasp.);并详细地对各类骨针化石进行了描述。虽然普通海绵骨针类型多样,但六射海绵的骨针丰度远高于普通海绵。简要地探讨了海绵骨针的保存方式,对比和分析了西蒿坪段和水井沱组海绵骨针化石组成的差异。结合同时代产自皖南荷塘组和云南澄江动物群中特异保存的海绵软躯体化石资料,认为虽然海绵动物起源于新元古代末期,但躯体海绵化石和骨针化石都显示海绵动物的大辐射事件发生在早寒武世筇竹寺期。     

生后雌性小鼠下丘脑室旁核内ER—β表达的免疫组化研究

研究发现小鼠下丘脑室旁核(PVN)内雌激素β受体(ER-β)的表达与在大鼠等一些实验动物脑PVN的表达有差异,提示其在小鼠PVN内的表达可能有特定的生理意义。为了深入探讨ER—β在小鼠PVN内的功能,本文采用硫酸镍铵增强显色的免疫组化SP法研究了ER—β在生后雌性小鼠PVN内的表达。结果发现ER—β免疫阳性物质主要见于PVN的大细胞部,在小细胞部和背侧帽部免疫阳性细胞数目较少。免疫阳性物质主要位于细胞核内,未发现明显的胞浆或突起阳性,但在发育的某些时期可见免疫阳性细胞核局部呈现阴性反应。最高表达见于生后早期(第1—9天),随后表达降低,生后一个月即达到成年水平。PVN内ER-β的表达模式表现为生后早期表达高、随后降低,提示在该部位ER—β可能主要参与了对生后早期PVN的神经内分泌活动以及神经结构的发育与完善的调控,并可能与生后早期动物的应激、体重增加和脂肪代谢等有关。     

Purification and in vitro cultivation of archaeocytes (stem cells) of the marine sponge <Emphasis Type="Italic">Hymeniacidon perleve</Emphasis> (Demospongiae)

Marine sponges (Porifera) are the best source of marine bioactive metabolites for drug discovery and development, although the sustainable production of most sponge-derived metabolites remains a difficult task. In vitro cultivation of sponge cells in bioreactors has been proposed as a promising technology. However, no continuous cell line has as yet been developed. Archaeocytes are considered to be toti/multipotent stem cells in sponges and, when purified, may allow the development of continuous sponge cell lines. As a prerequisite, we have developed a novel four-step protocol for the purification of archaeocytes from a marine sponge, Hymeniacidon perleve: (1) differential centrifugation to separate large sponge cells including archaeocytes; (2) selective agglomeration in low-Ca²⁺/Mg²⁺ artificial seawater in which living archaeocytes form small loose aggregates with some pinacocytes and collencytes; (3) differential adherence to remove anchorage-dependent pinacocytes, collencytes and other mesohyl cells; (4) Ficoll-Vrografin density gradient centrifugation to purify archaeocytes. The final purity of archaeocytes is greater than 80%. The proliferation potential of the archaeocytes has been demonstrated by high levels of BrdU incorporation, PCNA expression and telomerase activity. In 4-day primary cultures, the purified archaeocytes show a 2.5-fold increase in total cell number. This study opens an important avenue towards developing sponge cell cultures for the commercial exploitation of sponge-derived drugs. The authors are grateful for the financial support of the Chinese Academy of Sciences under the “100 Talent Project”, the “Innovation Fund” from the Dalian Institute of Chemical Physics, the “Hi-Tech Research and Development Program of China” (2001AA620404), and the European Commission (project: Silicon Biotechnology).     

Primary cell culture from the nose of a marine organism, the banded houndshark, Triakis scyllium

Animal cells have been widely and continuously studied due to their usefulness in biological researches and production of pharmacological agents as well as food additives. Nevertheless, there are several problems such as the existence of viruses which introduce the possibility of mammalian-infection. In this reason, recently, animal cells derived from marine organisms have emerged to overcome these problems by many researches. However, marine animal-derived cells have not yet been well developed. The banded hound shark occupies an important position in an evolutionary perspective and currently a few biological substances have been used for medicines or food additives such as shark squalene and cartilage extract. In this study, primary cells were cultivated from a banded hound shark nose containing many extracellular matrix (ECM) materials. After successful isolation of one type of primary nasal cell, we optimized culture conditions including coating materials, media composition, serum concentrations and pH. Additionally, these cells demonstrated proliferation ability in vitro, generating secretions of collagen and sulfated polysaccharides. The cultivated primary cells are useful in the study of cellular biology and may be used to create a variety of ECM-originated bioactive substances.     

Ultrastructural study of differentiation processes during aggregation of purified sponge archaeocytes

Archaeocytes from the spongeEphydatia fluviatilis were dissociated and then isolated on Ficoll density gradients. Their aggregation and reconstitution processes were studied by transmission electron microscopy to determine their capabilities for differentiation.Archaeocyte aggregates follow a well defined sequence of differentiation to generate the characteristic structures of a sponge. Pinacoderm is the first structure to be regenerated and appears progressively at the surface of the 12 h aggregates. Pinacocytes which have differentiated in archaeocyte aggregates are identical to native ones except that the nucleolus remains in most cells. The choanocytes appear only after 24 h by a two step process. First, small cells (choanoblasts) are formed from archaeocytes by mitosis. These cells then transform into fully differentiated choanocytes possessing collars and flagella. The early choanocyte chambers are small, irregular and randomly dispersed in the aggregates. Finally, collencytes and sclerocytes begin to appear just before the aggregates spread on the substrate.The differentiation of a suspension of pure archaeocytes is a unique model system to study sponge cell differentiation and has allowed us to demonstrate that archaeocytes isolated from developed sponges maintain the capacity to differentiate even though this capacity is not usually expressed.     

Cell cycle analysis of primary sponge cell cultures

Proliferation of sponge cells is generally measured via cell counts or viability assays. However, more insight into the proliferative state of a sponge cell population can be obtained from the distribution of the cells over the different phases of the cell cycle. Cell cycle distribution of sponge cells was measured via flow cytometry after staining the DNA with propidium iodide. The five sponges studied in this paper all showed a large fraction of cells in G1/G0 compared to G2/M and S, indicating that cells were not actively dividing. In addition, some sponges also showed a large apoptotic fraction, indicating cell death. Additional apoptosis measurements, based on caspase activity, showed that harvesting and dissociation of sponge tissue to initiate a primary cell culture was directly correlated with an increase in apoptotic cells. This indicates that for the development of cell cultures, more attention should be given to harvesting, dissociation, and quality of starting material. Finally, cultivation conditions used were ineffective for proliferation, since after 2 d of cultivating Haliclona oculata cells, most cells shifted towards the apoptotic fraction, indicating that cells were dying. For development of in vitro sponge cell cultures, flow cytometric cell cycle analysis is a useful method to assess the proliferative state of a sponge cell culture and can be used to validate improvements in harvesting and dissociation, to select sponges with good proliferative capacities and to study the influence of culture conditions for stimulating cell growth.     

Hydra size and budding rate: influence of feeding

Summary

In the present study of Dugesia tigrina, the development of the nervous system is followed and compared during regeneration after fission and after decapitation. Immunocytochemistry was used, with antisera raised against the biogenic mine, 5-hydroxyhyptamine (5-HT) and the two neuropeptides, neuropeptide F (NPF), and FMRFamide. The results indicate that two processes are involved in the formation of the new cerebral ganglion. First, new processes sprouting from the original main longitudinal nerve cords bend transversely, indicating the position of the developing horseshoe-shaped anterior cerebral commissure. Then new nerve cells in front of the commissure differentiate from neoblasts and their growth cones fasciculate with the fibres from the old main longitudinal nerve cords. In the cerebral ganglion, 5-HT-IR cells appear before NPF-IR cells, in contrast to the pharynx where NPF-IR cells differentiate before the 5-HT-IR cells. In the peripheral nervous system, NPF-IR fibres and cells appear at a very early stage and dominate the whole regeneration process. A role for the PNS in early pattern formation is suggested.     

Presence of cells and fibers immunoreactive toward antibodies to different peptides or amine in the digestive tract of the snailHelix aspersa

An immunocytological study of four different parts of the gut of Helix aspersa clearly demonstrates the presence of many cells and fibers immunoreactive toward antibodies directed to vertebrate (α, β-endorphin, α, β-MSH, ACTH 1–24 and ACTH 17–39, met-enkephalin, somatostatin, insulin, glucagon, P.P., serotonin) or invertebrate (FMRF-amide) peptides. These results are evidence of the presence of different substances related to known peptides or amines in the epithelial and connective tissue cells and nerve fibers of the snail gut. Immunocytochemistry may help to elucidate the morpho-functional characteristics of the enteroendocrine cells of H. aspersa.     

Origin of neuronal-like receptors in Metazoa: cloning of a metabotropic glutamate/GABA-like receptor from the marine sponge Geodia cydonium

To date, no conclusive evidence has been presented for the existence of neuronal-like elements in Porifera (sponges). In the present study, isolated cells from the marine sponge Geodia cydonium are shown to react to the excitatory amino acid glutamate with an increase in the concentration of intracellular calcium [Ca2+]i. This effect can also be observed when the compounds L-quisqualic acid (L-QA) or L-(+)-2-amino-4-phosphonobutyric acid (L-AP-4) are used. The effect of L-QA and L-AP-4, both agonists for metabotropic glutamate receptors (mGluRs), can be abolished by the antagonist of group I mGluRs, (RS)-alpha-methyl-4-carboxyphenylglycine. These data suggest that sponge cells contain an mGluR-like protein. A cDNA encoding rat mGluR subtype 1 has been used to identify the complete nucleotide sequence of G. cydonium cDNA coding for a 528-amino-acid-long protein (59 kDa) that displays marked overall similarity to mGluRs and to gamma-aminobutyric acid B receptors. The deduced sponge polypeptide, termed putative mGlu/GABA-like receptor, displays the highest similarity to the two families of metabotropic receptors within the transmembrane segment. The N-terminal part of the sponge sequence shows similarity to mGluR4 and mGluR5. These findings suggest that the earliest evolutionary metazoan phylum, the Porifera, possesses a sophisticated intercellular communication and signaling system, as seen in the neuronal network of higher Metazoa.     

Distribution of brominated compounds within the sponge<Emphasis Type="Italic"> Aplysina aerophoba</Emphasis>: coupling of X-ray microanalysis with cryofixation techniques

The major secondary metabolites of the sponge Aplysina aerophoba are brominated compounds. X-ray energy dispersive microanalysis was therefore used to locate secondary metabolites via the Br signal in energy emission spectra from sponge sections. To test the reliability of this method in the face of the loss or redistribution of metabolites during processing, we compared the results obtained by conventional aldehyde fixation with those obtained by cryofixation and cryosubstitution with and without cryoembedding. Bromine appeared to be concentrated in two sponge structures, viz. fibres and spherulous cells, when cryofixed material was examined. However, X-ray microanalysis failed to demonstrate the presence of bromine in spherulous cells in chemically fixed samples, showing the need for cryotechniques to avoid the loss of compounds. Cryofixation plus cryosubstitution methods performed best regarding structural preservation and the immobilization of metabolites. The presence of bromine in the spherulous cells suggests that this cell type is the producer of the secondary metabolites, as described for other sponge species. Nevertheless, the presence of bromine in sponge fibres indicates that they can accumulate metabolic substances, although we have been unable to assess whether the chemicals are in their original form or in a modified state within the fibres. A. aerophoba has both bacterial and cyanobacterial symbionts in its mesohyl; the absence of brominated compounds in them contrasts with previous findings in other sponges with prokaryote symbionts.     

Landscape connectivity of Cercidiphyllum japonicum,an endangered species and its implications for conservation

Cercidiphyllum japonicum, a Tertiary relict, recolonized areas north of the Yangtze River after the last glacial; however, little is known about its specific colonization corridors. Together with distribution models, the least cost path (LCP) analysis has been used to reveal the landscape connectivity of species. In this study, we utilized the categorical LCP method, combining the species distribution with genetic data from cpDNA and nuclear markers, to identify the possible dispersal routes of C. japonicum after the LGM. Across time periods and genetic markers, the results revealed that the species generally spread from the western edge of the Sichuan Basin, while the highest degree of dispersal potential corresponds with the year 2080 and the cpDNA haplotype. Furthermore, shifts in the species' range and the indication of an area of low genetic divergence further support the existence of a dispersal corridor. Overall, we believe that a dispersal route from the western edge of the Sichuan Basin through the Qinling Mountains and further to the northeast could exist, and therefore, the results are an important supplement to the evolutionary history of C. japonicum. In the future, we believe species distribution models (SDM) and connectivity assessment in relation to climate change will provide increasingly useful information and new implications for prioritizing the conservation of the endangered species.     

Immunocytochemistry of glutathione S-transferase in taste bud cells of rat circumvallate and foliate papillae

Immunocytochemistry was used to investigate the distribution of cells reacting with specific antibodies against glutathione S-transferase (GST) mu and pi in rat circumvallate and foliate taste buds; the findings were confirmed by Western blotting. Double immunofluorescence staining for protein gene product (PGP) 9.5 and GST subunits allowed the classification of taste bud cells of both papillae into: (i) cells immunoreactive to either PGP 9.5 or GST subunit antibody; (ii) cells immunoreactive to both antibodies; and (iii) cells that did not react with either of these antibodies. Immunoelectron microscopy revealed that most GST subunit-immunoreactive cells seemed to be either type II or type III cells based on their ultrastructure. Since PGP 9.5 is now widely used as a marker for type III cells in mammalian taste buds, it seems reasonable to believe that most GST subunit-immunoreactive cells are type II cells. Whether cells immunoreactive for both PGP 9.5 and GST subunits constitute a small subpopulation of type III cells or whether they are intermediate forms between type II and III cells is under investigation. No type I cells reacted with antibodies against GST subunits in the present study. GST subunits in taste bud cells may participate in xenobiotic metabolism of certain substances exposed to taste pits, as already shown for olfactory epithelium.